Detection of Antibodies to a Pathogenic Mycoplasma in American Alligators (Alligator mississippiensis), Broad-Nosed Caimans (Caiman latirostris), and Siamese Crocodiles (Crocodylus siamensis)

doi:10.1128/JCM.39.1.285-292.2001

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Journal of Clinical Microbiology, January 2001, p. 285-292, Vol. 39, No. 1
0095-1137/01/$04.00+0 DOI: 10.1128/JCM.39.1.285-292.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Detection of Antibodies to a Pathogenic Mycoplasma in American Alligators (Alligator mississippiensis), Broad-Nosed Caimans (Caiman latirostris), and Siamese Crocodiles (Crocodylus siamensis)

D. R. Brown,¹^,^* I. M. Schumacher,²^, M. F. Nogueira,¹^, L. J. Richey,¹ L. A. Zacher,¹ T. R. Schoeb,¹ K. A. Vliet,³ R. A. Bennett,⁴ E. R. Jacobson,⁴ and M. B. Brown¹

Department of Pathobiology,¹ Interdisciplinary Center for Biotechnology Research,² Department of Zoology,³ and Department of Small Animal Clinical Sciences,⁴ University of Florida, Gainesville, Florida 32611-0880

Received 26 June 2000/Returned for modification 4 September 2000/Accepted 19 October 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

An epidemic of pneumonia with fibrinous polyserositis and multifocal arthritis emerged in captive American alligators (Alligatormississippiensis) in Florida, United States, in 1995. Mycoplasmaalligatoris sp. nov. was cultured from multiple organs, peripheralblood, synovial fluid, and cerebrospinal fluid of affected alligators.In a subsequent experimental inoculation study, the Henle-Koch-Evanspostulates were fulfilled for M. alligatoris as the etiologicalagent of fatal mycoplasmosis of alligators. That finding was remarkablebecause mycoplasmal disease is rarely fatal in animals. An enzyme-linkedimmunosorbent assay (ELISA) for the detection of antibodies producedby alligators in response to M. alligatoris exposure was developedby using plasma obtained from naturally infected alligators duringthe original epidemic. The assay was validated by using plasmaobtained during an experimental dose-response study and appliedto analyze plasma obtained from captive and wild crocodilian species.The ELISA reliably detected alligator seroconversion (P < 0.05)beginning 6 weeks after inoculation. The ELISA also detected seroconversion(P < 0.05) in the relatively closely related broad-nosed caimanCaiman latirostris and the relatively distantly related Siamesecrocodile Crocodylus siamensis following experimental inoculationwith M. alligatoris. The ELISA may be used to monitor exposureto the lethal pathogen M. alligatoris among captive, repatriated,and wild crocodilianspecies.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

An epidemic of mycoplasmosis emerged in a collection of American alligators (Alligator mississippiensis) in Florida in 1995(4, 8). Thirty-three 200- to 300-kg adult male alligatorsdied, and 13 moribund alligators were euthanatized within 1 monthof the index case. Lesions observed at necropsy ranged from mildinterstitial and peribronchiolar pneumonia to fibronecrotic pneumonia.Extrapulmonary complications included pericarditis, myocarditis,and multifocal arthritis. Mycoplasma alligatoris proposed sp.nov. was isolated from multiple tissues, blood, synovial fluid,and cerebrospinal fluid of affected alligators. In a pilot experimentalinoculation study (5, 6), healthy alligators were inoculatedwith M. alligatoris strain A21JP2^T (ATCC 700619) to reproduce the disease and fulfill the Henle-Koch-Evanspostulates (11) for M. alligatoris as the etiological agentof synovitis, polyserositis, and pneumonia of alligators. Theresults were remarkable because, except for bovine and caprinepleuropneumonia, mycoplasmal disease is rarely fatal inanimals.

The origin of the 1995 epidemic remains unknown, but the disease may emerge under conditions of captivity. Crocodilians arefrequently sold or traded among collections, exhibits, zoos, andranches. Many collections include multiple species of crocodilians.Some crocodilians from commercial ranches are repatriated after"head-starting" hatchlings from eggs collected in the wild, apotential vector for catastrophic infection of wild populationsif lethal disease emerges in captivity. A validated serodiagnostictool could be used to test captive crocodilians for exposure toM. alligatoris and prevent spread of the pathogen. The objectiveis to ensure that crocodilians used for commercial purposes orreturned to the wild are free of the pathogen. In this report,we describe the development, validation, and application of anenzyme-linked immunosorbent assay (ELISA) for the detection ofantibodies to M. alligatoris in alligators, caimans, andcrocodiles.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Antigen preparation. M. alligatoris strain A21JP2^T was cloned from a single colony isolated from limb joint synovial fluid of an American alligatorthat died during a 1995 epidemic (6). Whole-cell lysate antigen(16) was prepared from a 1-liter culture of third-passage M.alligatoris A21JP2^T grown at 30°C in ATCC medium 988 broth (SP4 [40]) supplementedwith 20% (vol/vol) fetal bovine serum (Gibco, Grand Island, N.Y.).The protein concentration was determined colorimetrically (Bio-Rad,Hercules, Calif.) and adjusted to 100 µg/ml, and the antigen wasstored at $-$ 70°C in polypropylenecryovials.

Whole-cell lysate antigen was similarly prepared from Mycoplasma bovis ATCC 25523, Mycoplasma iowae ATCC 33552, Mycoplasmamicroti ATCC 700935, Mycoplasma pulmonis ATCC 19612, and mycoplasmasisolated from other reptiles, including Mycoplasma agassizii ATCC700616, Mycoplasma crocodyli ATCC 51981, Mycoplasma testudinisATCC 43263, two isolates of the unnamed mycoplasma ATCC 700618from tortoises, and Acholeplasma laidlawii isolated from a tortoise(3). Those mollicutes were grown in SP4 supplemented with fetalbovine serum or Frey's medium (40) supplemented with horse serum(Gibco).

Antigen enriched for lipid-associated membrane proteins (LAMP) was prepared from a 1-liter culture of third-passage M. alligatorisA21JP2^T grown at 30°C in SP4 broth supplemented with 20% fetal bovineserum by Triton X-114 phase fractionation (14). The proteinconcentration was adjusted to 100 µg/ml, and the antigen was storedat $-$ 70°C in polypropylene cryovials. A LAMP-enriched antigen wassimilarly prepared from M. agassizii.

Crocodilian plasma samples. Blood samples were collected from the supravertebral sinus into glass tubes containing lithium heparin anticoagulant (BectonDickinson, Rutherford, N.J.). Plasma was separated by low-speedcentrifugation. All plasma samples were stored at $-$ 70°C in polypropylenecryovials until the analyses wereperformed.

Plasma samples were obtained from 40 naturally exposed alligators during the 1995 epidemic. In a pilot experimental inoculationstudy, healthy juvenile (approximately 1 m long) alligators wereinoculated by intracoelomic injection (n = 2) or by instillationthrough the glottis (n = 2) with 10⁶ CFU of M. alligatoris strain A21JP2^T in 1 ml of SP4 broth. A control alligator received sterile broth.Plasma samples were collected at weekly intervals until the alligatorseither died or were euthanatized 14 weeks postinoculation (w.p.i.).In a follow-up experimental dose-response study, healthy youngadult (approximately 1.5 to 2 m long) female alligators were inoculatedby instillation through the glottis with 10², 10⁴, or 10⁶ CFU (six per treatment) of M. alligatoris strain A21JP2^T in 1 ml of SP4 broth. Four controls received sterile SP4 brothor no treatment. Plasma samples were collected at weekly intervalsfor 4 weeks and then biweekly until the alligators either diedor were euthanatized at 12 to 16 w.p.i. In an experimental hostrange study conducted concurrently with the dose-response study,six each of healthy young adult female broad-nosed caimans (Caimanlatirostris) and Siamese crocodiles (Crocodylus siamensis) wereinoculated by instillation through the glottis with 10⁶ CFU of M. alligatoris strain A21JP2^T in 1 ml of SP4 broth. Controls (two per species) received sterileSP4 broth. Plasma samples were collected at weekly intervals for4 weeks and then biweekly until the crocodilians either died orwere euthanatized at 12 to 16 w.p.i. Plasma samples were alsoobtained during routine health assessment of 70 American alligatorsin captivity at the Silver Springs Wildlife Park (Ocala, Fla.);29 Siamese crocodiles in captivity at the Sriracha Crocodile Farm(Sriracha, Thailand), and 42 wild American crocodiles (Crocodylusacutus) inBelize.

Conjugate. Proteins were precipitated from a pool of American alligator plasma samples by adding ammonium sulfate to a concentrationof 25% (wt/vol) and dissolved in 10 mM 2-(N-morpholino)ethanesulfonicacid, pH 5.5. The proteins were fractionated by ion-exchange chromatographyon mixed-resin silica gel (Bakerbond ABX Antibody Exchanger; MallinckrodtBaker, Phillipsburg, N.J.) using a gradient of 0 to 100% elutionbuffer (500 mM ammonium sulfate, 20 mM sodium acetate). Columnfractions enriched for immunoglobulins (Ig) were identified bypredominant Coomassie-stained bands of approximately 28 kDa, consistentwith reptile Ig light chain, and approximately 60 kDa, consistentwith reptile IgY heavy chain (36, 37), after denaturing 12.5%polyacrylamide gel electrophoresis (PAGE; PhastGel System; Pharmacia,Piscataway, N.J.). The Ig were purified by column filtration onSephacryl S-300 gel (Pharmacia), and purity was reconfirmed byPAGE. Rabbit antiserum against the purified alligator Ig was preparedby using standard immunization methods (Pel-Freez Biologicals,Rogers, Ark.). Polyclonal anti-alligator Ig antibodies were purifiedfrom rabbit serum by affinity column chromatography (HiTrap ProteinG; Pharmacia) and then conjugated with biotin (EZ-Link Sulfo-NHS-LCbiotin; Pierce, Rockford, Ill.).

To determine the relative avidity of the conjugate, each well of a 96-well flat-bottomed microplate (Nunc-Immuno MaxiSorp;Nunc, Kamstrup, Denmark), excluding the perimeter wells, was coatedwith 50 µl of healthy American alligator (n = 2), broad-nosedcaiman (n = 2), or Siamese crocodile (n = 2) plasma serially dilutedfrom 1:2 to 1:1,024 in PBS/A (sodium phosphate buffer [pH 7.2]containing 0.15 M NaCl and 0.02% NaN₃) by incubating overnightat 4°C in a sealed humidified container. The wells were washedfour times with 350 µl of PBS/A containing 0.05% Tween 20 (PBS/T)by using an automatic microplate washer (EL 403H; Bio-Tek Instruments,Winooski, Vt.) and then blocked with 250 µl per well of PBS/Tcontaining 5% (wt/vol) nonfat dry milk (PBS/TM) overnight at 4°C.After four more washes, 50 µl of biotinylated polyclonal anti-alligatorIg (approximately 150 ng of protein) diluted in PBS/TM was added.The microplate was incubated at room temperature for 60 min ona nutator and washed as described above, and then 50 µl of alkalinephosphatase-conjugated streptavidin (Roche, Indianapolis, Ind.)diluted 1:1,000 in PBS/TM was added to each well. The microplatewas incubated and washed as described above, and then 100 µl ofp-nitrophenyl phosphate disodium (1 mg/ml in 0.01 M sodium bicarbonate[pH 9.6], 2 mM MgCl₂) was added to each well. The microplate wasthen incubated in the dark without agitation at room temperature.The A₄₀₅ of each well was measured after 30 min (Thermomix microplatereader with Softmax Pro version 1.2.0 software; Molecular Devices,Sunnyvale, Calif.). Cross-reactivity with plasma available fromChinese alligator (Alligator sinensis), black caiman (Melanosuchusniger), American crocodile, Morelet's crocodile (Crocodylus moreletii),Nile crocodile (Crocodylus niloticus), Australian saltwater crocodile(Crocodylus porosus), Cuban crocodile (Crocodylus rhombifer),and false gavial (Tomistoma schlegelii) was alsoevaluated.

Immunoblotting. The specificities of the polyclonal anti-alligator Ig were demonstrated by Western immunoblotting. Samples of plasma fromhealthy alligators, caimans and crocodiles were diluted 1:50 inPBS/A and then separated by PAGE under denaturing conditions witha precast 10% (bis-Tris)polyacrylamide gel and MOPS (morpholinepropanesulfonicacid) running buffer (NuPAGE; Novex, San Diego, Calif.). The separatedproteins were electroblotted by standard methods from the gelonto a nitrocellulose membrane, which was then blocked with PBS/TMovernight at 4°C. The blocked blot was washed with PBS/T and thenincubated in purified but unbiotinylated polyclonal anti-alligatorIg (1 µg/ml in PBS/A) for 60 min at room temperature with agitation.After washing, the membrane was incubated in alkaline phosphatase-conjugateddonkey anti-rabbit Ig (diluted 1:10,000 in PBS/TM; Pierce) for60 min at room temperature with agitation. After the final wash,the blot was developed in substrate buffer (0.1 M Tris-HCl [pH8.8], 1 mM MgCl₂) containing nitroblue tetrazolium chloride and5-bromo-4-chloro-3-indolylphosphate p-toluidine salt (Life Technologies,Grand Island, N.Y.).

Western immunoblots of whole-cell lysate and LAMP-enriched antigen preparations used for ELISA were similarly prepared. Antigensbound by specific antibodies in pooled seropositive alligator,caiman, and crocodile plasma (see below) were detected by usingthe polyclonal anti-alligator Ig and alkaline phosphatase-conjugateddonkey anti-rabbit Ig as describedabove.

Determination of ELISA parameters. Plasma samples obtained from the pilot experimental inoculation study served as positive and negative specimens to establishreaction conditions for a preliminary ELISA. The titer (heuristicallydefined as the highest plasma dilution with an A₄₀₅ more thantwice that of the negative control) of plasma obtained from alligatorsduring the 1995 epidemic was determined by using whole-cell lysateantigen. Selected samples were then pooled to create high-range(titer, 1:5,120), midrange (titer, 1:1,280), and low-range (titer,1:80) plasma pools used in the final ELISAvalidation.

ELISA procedure. The A21JP2^T whole-cell lysate or LAMP-enriched antigen was thawed, passed several times through a 30-gauge needle, and thendiluted to 15 µg/ml in PBS/A. Each microplate well, excludingthe perimeter wells, was coated with 50 µl of antigen and thenwashed and blocked as described above. After four washes, 50 µlof crocodilian plasma diluted 1:1,000 in PBS/TM was added in duplicate,and the microplate was incubated at room temperature for 60 minon a nutator. From this point forward, the assay was as describedabove for conjugate validation. On each microplate, the backgroundwas the mean A₄₀₅ of duplicate wells processed identically tothe sample wells except without plasma. The background absorbancewas subtracted from the measured A₄₀₅ of each well before dataanalyses. Each microplate also included duplicate high-range,midrange, and low-range alligator plasma poolstandards.

Binding of antibody in alligator plasma to whole-cell lysate or LAMP-enriched antigens prepared from the other mollicuteslisted above was also assayed in the ELISA format described. Controlwells were coated with culture medium with and without fetal calfor horseserum.

Within-batch and between-batch assay variability was assessed by using the Youden plot graphic method (17). The ELISA valuesobtained for the high-range, midrange, and low-range plasma poolstandards included on each microplate coated with whole-cell lysatewere used to establish target values and control limits to beused for monitoring the consistency of the assay (10 batches).The values obtained for each standard at the beginning of a seriesof assays were plotted against the values obtained for the samestandards at the end of the series. Imprecision was shown by randomdeviations at right angles to the slope formed by the expectedvalues, and drift was indicated if all deviations were in thesame direction at right angles to theslope.

Statistical analyses. Data from the dose-response study and the host range study were combined for statistical analysis. Seroconversion was determinedby repeated-measure analysis of variance with main effects ofw.p.i., species, and treatment group within species. Fisher'sprotected least significant difference (LSD) was used for posthoc comparisons if main effects were significant. A P value of< 0.05 was consideredsignificant.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Controlling the spread of mycoplasmal infections among captive animals such as swine, poultry, and laboratory rodents dependsprimarily on identification of individuals whose exposure to thepathogen is indicated by the presence of specific antibody. Themost commonly used serological test to diagnose mycoplasmal infectionsis the ELISA, which is amenable to automation and stringent qualitycontrols. The rationale of the experiments described was to developreagents and a protocol for an ELISA which could be used to controlthe spread of M. alligatoris, the newly recognized lethal mycoplasmalpathogen of alligators, amongcrocodilians.

Conjugate avidity and specificity. The relative avidity and specificity of the biotinylated polyclonal anti-alligator Ig antibody used in the ELISA was comparedamong alligator, caiman, and crocodile Ig. The results of conjugatebinding to serially diluted plasma from each species coated directlyin ELISA microplate wells are shown in Fig. 1. Crocodiles arerelatively phylogenetically distant from alligators and caimansbut the avidity of the polyclonal antibody was only slightly lowerfor Siamese crocodile Ig than for alligator Ig. Avidity for broad-nosedcaiman Ig was about twofold higher than for alligator Ig. Thoseresults demonstrated that same-species control plasma should beused for diagnostic crocodilian ELISA. The conjugate also cross-reacted(minimum titer, 1:>10) in similar assays with plasma availablefrom the other crocodilian species listed above (data not shown).

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FIG. 1. Relative avidity of polyclonal rabbit anti-alligator Ig antibodies for Ig from healthy crocodilians measured by ELISA. Serially diluted plasma from pools of each species was coated directly in microplate wells, and conjugate binding was measured under conditions used for the diagnostic ELISA. Avidity for crocodile Ig was slightly lower and for caiman Ig was about twofold higher than for alligator Ig.

The specificity of the polyclonal anti-alligator Ig antibody for crocodilian plasma proteins separated by denaturing PAGEis shown in Fig. 2. The two predominant bands recognized in alligatorand crocodile plasma had apparent sizes of approximately 28 kDa,consistent with reptile Ig light chain, and approximately 55 kDa,consistent with reptile IgY heavy chain (36, 37), on the 10%polyacrylamide gel. Other bands detected may represent incompletelydenatured IgY, IgM heavy chain, or antibodies against contaminantsremaining in the plasma fraction used for immunization. The twopredominant bands recognized in caiman plasma consistently appearedto be slightly larger and smaller, respectively, than those inalligator and crocodile plasma.

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FIG. 2. Western immunoblot of polyclonal rabbit anti-alligator Ig binding to pooled plasma from healthy crocodilians. Lanes (left to right): prestained molecular mass standards, alligator plasma, caiman plasma, and crocodile plasma. The predominant bands recognized by the conjugate, which was used as the secondary antibody in the ELISA, are consistent with reptile 28-kDa Ig light chain and 55-kDa IgY heavy chain separated on a denaturing 10% polyacrylamide gel. The predominant bands recognized in caiman plasma were consistently slightly different in size from those in alligator and crocodile plasma.

ELISA development. In the pilot experimental inoculation study, three of four inoculated alligators died between 1 and 3 w.p.i. before seroconversion.Plasma obtained at necropsy at 14 w.p.i. from the one survivinginoculated alligator (titer, 1:640) and from the uninoculatedcontrol (titer, 1:<10) were the only specimens obtained undercontrolled conditions which could serve as positive and negativespecimens, respectively, to establish the preliminary ELISA conditions.Once those were optimized, it was important to test standardswhich produced a wide range of absorbance values, to determinewhat sample dilution should be used for a single-dilution ELISA.A sample dilution of 1:1,000 gave absorbance readings within thelinear response to dilution of the high-range, midrange, and low-rangeplasma pool standards and the microplate reader under the assayconditions described (Fig. 3).

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FIG. 3. Sample dilution validation. Serial dilutions of pools of alligator plasma with high-range (1:5,120), midrange (1:1,280), and low-range (1:80) titers were assayed by ELISA using whole-cell lysate antigen. A dilution of 1:1,000 gave absorbance readings within the linear response to dilution of each pool under the assay conditions described.

Coomassie staining of antigens separated by sodium dodecyl sulfate-PAGE showed that about 10% of total M. alligatoris proteinremained in the LAMP-enriched fraction. That value was consistentwith the total protein yields for whole-cell lysate and LAMP preparationsfrom equal volumes of broth cultures. The Western immunoblot patternsof antigens used in the ELISA are shown in Fig. 4. The majorityof the antigens recognized on immunoblots of whole-cell lysatewere present in the LAMP-enriched fraction. Antigens recognizedby caiman and crocodile antibodies were a subset of those recognizedby alligator antibodies.

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FIG. 4. (A) PAGE of Coomassie-stained M. alligatoris proteins used as ELISA antigens. Lanes (left to right): prestained molecular mass standards, whole-cell lysate, and LAMP-enriched fraction. The LAMP proteins, prepared by Triton X-114 phase fractionation, were a minor proportion of total cellular protein. (B) Western immunoblot of M. alligatoris whole-cell lysate antigen probed with seropositive (left to right) alligator plasma, caiman plasma, and crocodile plasma. Antigens recognized by caiman and crocodile antibodies were a subset of those recognized by alligator antibodies. (C) Western immunoblot of M. alligatoris LAMP antigen probed with seropositive (left to right) alligator plasma, caiman plasma, and crocodile plasma. The majority of antigens recognized in immunoblots of whole-cell lysate were LAMP antigens.

The between-batch bias control limits were established at 26% above and below the target value for the low-range standard(mean A₄₀₅ = 0.167 ± 0.030 [standard error (SE)]; coefficent ofvariation [CV] = 0.181) and 18% above and below the midrange (meanA₄₀₅ = 0.676 ± SE 0.081, CV = .120) and high-range (mean A₄₀₅= 1.493 ± SE 0.159, CV = 0.106) standards. The drift control limitswere established at angles 4° (11%) above and below the slopeof the target values. The control limits are statistically arbitrary(17).

Detection of crocodilian seroconversion by ELISA. Three alligators inoculated with 10⁶ CFU and two caimans died within 4 w.p.i. and a third caiman died 10 w.p.i. during thedose-response and host range studies. Mycoplasmas were culturedquantitatively in high numbers from trachea, lung, coelomic cavity,liver, spleen, interior of pericardial sac, heart, blood, limbjoints, and brain of those crocodilians. Mycoplasmas were notcultured at any time point from the remaining three highest-dosealligators and caimans, alligators inoculated with 10⁴ or 10² CFU, or any of the negative controls. Mycoplasmas were culturedat necropsy in small numbers from a single site, the tonsils,of three inoculated crocodiles. The identity of the mycoplasmasreisolated from each individual was confirmed by restriction endonucleaseanalyses of the PCR-amplified mycoplasmal 16S rRNA gene. OnlyM. alligatoris was recovered. Together, those findings indicatedthat the culture methods employed in this study did not detectany mycoplasmas among the normal flora ofcrocodilians.

Plasma obtained during the dose-response and host range studies was used to validate the ELISA. Seroconversion was definedas a statistically significant increase in A₄₀₅ value from thepreinoculation group mean and from the same-species negative controlmean. In all groups inoculated with 10⁶ CFU of M. alligatoris, seroconversion (P < 0.05) was detectablebeginning 6 to 8 w.p.i. when whole-cell lysate antigen was used(Fig. 5). For all groups, the minimum statistically significantincrease was to A₄₀₅ values about two times those of preinoculationor negative control means. That value was in remarkably good agreementwith the cutoff between positive and negative results in the onlyother validated reptile mycoplasmosis ELISA (36) and with thevalue used heuristically to determine positive-control pool titers.When M. alligatoris LAMP-enriched antigen was used in the ELISA,crocodile seroconversion was also evident by 6 w.p.i., but increasesin specific antibody in alligators were not statistically significant,and caiman plasma showed no measurable binding to LAMP-coatedplates whatsoever (Fig. 6).

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FIG. 5. Seroconversion assayed by whole-cell lysate antigen-based ELISA. Each species (n = 6) was inoculated with 10⁶ CFU of M. alligatoris. Seroconversion was determined by repeated-measure analysis of variance with main effects of week and species. Fisher's protected LSD was used for post hoc comparisons if main effects were significant. Time points at which species means differed (P < 0.05) from preinoculation and from same-species negative controls (data for control alligators are shown in Fig. 7; two controls per species for caiman and crocodiles [data not shown]) are indicated by asterisks. Statistical power to detect seroconversion of alligators and caimans was reduced at later time points because some individuals in those groups succumbed to mycoplasmosis.

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FIG. 6. Crocodile seroconversion assayed by LAMP antigen-based ELISA. Each species (n = 6) was inoculated with 10⁶ CFU of M. alligatoris. Seroconversion was determined by repeated-measure analysis of variance with main effects of week and species. Fisher's protected LSD was used for post hoc comparisons if main effects were significant. Time points at which the inoculated crocodile group mean differed (P < 0.05) from preinoculation and from the negative control crocodiles (n = 2; data not shown) are indicated by asterisks. Changes from preinoculation and from negative controls (four alligators and two caimans) in alligators and caimans were not significant. Statistical power to detect seroconversion of alligators and caimans was reduced at later time points because some individuals in those groups succumbed to mycoplasmosis.

The rate of seroconversion was consistent with the rate of specific antibody response of other reptiles to experimental mycoplasmosis(7) and of alligators to experimental immunization with otherantigens (21). However, the magnitude of the specific antibodyresponse of alligators inoculated with M. alligatoris in the dose-responsestudy was lower than that observed in plasma from the 1995 epidemic.The magnitude of response was higher (P < 0.05) for crocodilesthan for caimans (Fig. 5), even without adjustment for apparentdifferences in conjugate avidity. The statistical power to detectseroconversion of alligators inoculated with 10⁶ CFU and of caimans later than 3 w.p.i. was reduced because thespecific antibodies developed too slowly to be detected beforehalf of the individuals in those groups died. Trends toward seroconversionin alligators inoculated with 10⁴ or 10² CFU were not statistically significant (Fig. 7).

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FIG. 7. Alligator seroconversion assayed by whole-cell lysate antigen-based ELISA. Alligators (six per group) were inoculated with 10² (low-dose), 10⁴ (middose), or 10⁶ (high-dose) CFU of M. alligatoris. Seroconversion was determined by repeated-measure analysis of variance with main effects of week and dose. Fisher's protected LSD was used for post hoc comparisons if main effects were significant. Time points at which dose group means differed (P < 0.05) from preinoculation and from the negative control alligators (n = 4) are indicated by asterisks. Seroconversion of the high-dose group was evident by 6 w.p.i. (same data shown in Fig. 5), but statistical power at later time points was reduced because some individuals in that group succumbed to mycoplasmosis. No meaningful trend toward seroconversion was detected for the low-dose or middose groups.

Binding to other antigens. Binding of antibody in standard pools of alligator plasma to whole-cell lysate or LAMP-enriched antigens of other mollicutesin the ELISA format is shown in Fig. 8. A gradient of cross-reactivitywas observed, but there was no consistent relationship to thesource of the other mollicutes (reptile versus avian or mammalianhosts) or to their position in the phylogeny of mollicutes basedon 16S rRNA gene nucleotide sequences (23). The maximum amountof binding that could be attributed to reactivity of alligatorplasma or polyclonal rabbit anti-alligator Ig antibody with culturemedium components was 0.05 A₄₀₅ unit.

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FIG. 8. Cross-reactivity of alligator plasma pools with high-range (1:5,120), midrange (1:1,280), and low-range (1:80) anti-M. alligatoris titers with whole-cell lysate or LAMP antigens of other mollicutes assayed by ELISA. No relationship to the mollicutes' usual hosts (reptile, avian, or mammalian) or to their position in the phylogeny of mollicutes based on 16S rRNA gene sequences was observed.

Survey for M. alligatoris-specific antibodies in captive crocodilians. The validated ELISA was used to analyze plasma obtained during routine health assessments of American alligators in captivityin the United States, American crocodiles being collected in Belize,and Siamese crocodiles in captivity in Thailand. The clinicalhealth status of all of those crocodilians was normal, and therewas no known history of mycoplasmosis or unexplained morbidityin those groups. All samples were seronegative (A₄₀₅ values lessthan two times that of the same-genus negative control). Thoseresults were further support for the conclusion that mycoplasmasare not commonly found among the normal flora of crocodiliansand indicated that the risk of false-positive ELISA results islow.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Epidemiology and control of crocodilian diseases are issues of broad significance to protection of many species, alternativecommodity production, and wetland conservation. Commercial useof alligators illustrates the potential significance of M. alligatorispathogenesis and the need for a diagnostic test. Ranching of Americanalligators is an alternative commodity industry in the U.S. GulfCoast states. More than 100 ranches annually produce approximately150,000 hides and 330,000 kg of meat, worth in excess of $75 millionto $150 million, from approximately 175,000 alligators. The ranchingof crocodilians for commercial production of hides and meat isan international industry, and live alligators are exported fromthe United States. In the 1990s, there were more than 600 ranchesin 47 countries, with annual stock in excess of 1.1 million crocodilians.American alligators are the most commonly ranched species, withabout 500,000 held in production facilities. Annual alligatorhide production outside the United States exceeds 182,000. Theannual world market is approximately 2 million crocodilianhides.

The crocodilian ranching industry is based on collection of eggs and hatchlings from the wild. By deriving an economic valuefrom those animals, individuals and governments are encouragedto protect not only the crocodilian populations but also the wetlandsnecessary for the continued survival and reproduction of the species.Commercial ranching operations thus are closely tied to the healthand productivity of wild crocodilian populations. For that reason,some wild populations are intermittently replenished with juvenilecrocodilians repatriated from commercial ranches after "head-starting"hatchlings from eggs collected in the wild. That practice couldprovide a vector for infectious disease transmission which mightbe interrupted by appropriate serologicalscreening.

Several features of reptile immunity present special challenges to diagnosis of infection by measuring seroconversion (1).Specific immunity begins with maternal antibodies present in reptileegg yolk (24, 37). Ontogenic maturation of immune system cellsprogresses slowly in some species, with full immune competencenot reached until months after hatching, but other species seemto be immunocompetent at hatching (10). Body temperature canhave a direct effect on reptile immune systems, with species-specificoptima and compromised immunity at body temperature extremes (9,39). The spleen, thymus, and gut-associated lymphoid tissuesof many reptiles undergo marked seasonal involutions (12, 43).That cycle seems to coincide with neuroendocrine rhythms correlatedwith mating periods (33, 34), independent of the direct effectsof body temperature. Compromised immunity, including inhibitedB-cell proliferation and differentiation and low antibody titers,was correlated with seasonal high levels of corticosteroids andsex steroids in several species of reptiles (20, 32, 43).The effects of each of those classes of hormones on immunity maybe independent, as has been investigated by administration ofexogenous testosterone (34) or hydrocortisone (33) or by pharmacologicaladrenalectomy (33). Consistent with those observations, sexualdimorphism in reptile immune responses has also been reported,with males having a somewhat delayed and less vigorous responseand significantly lower antibody titers than females in responseto immunization during seasons when testosterone is significantlyhigher in males (31, 35). The B-cell inhibition observed maybe due in part to lack of T-cell-derived lymphokines, becausestrong cell-mediated immune responses coincide with seasons duringwhich lymphoid tissue is well developed. However, seasonal effectson responses to immunization with a T-cell-independent antigenhave also been observed (11). Thus, potential influences ofage, temperature, season, and hormones on immunity should be consideredwhen attempting to interpret the results of serological testssuch as ELISA to diagnose infection in reptiles. The majorityof the alligators that died during the 1995 epidemic were >200-kgadult males which died in September and October, while the alligatorsused in the pilot inoculation and dose-response studies were <20-kgyoung adult females which were inoculated in June. Those age,season, and sex differences may account for the somewhat lesspronounced antibody responses observed in thosestudies.

It is unlikely that the less pronounced antibody response observed in alligators in the pilot inoculation and dose-responsestudies was because the M. alligatoris had attenuated immunogenicity(without loss of virulence) after clonal isolation and laboratorypassage. Many mycoplasmal species exhibit extensive intraspeciesphenotypic variability, manifested as antigenic variation in thecontext of immune recognition by infected hosts, so mycoplasmasare almost always very immunogenic (42). The antigenic variationcan be apparent even among successive isolates obtained from aninfected individual (22, 28). The variation probably providesthe mycoplasmas with flexibility in interacting with their environmentand may contribute to host specificity, pathogenicity, and evasionof host defenses (30, 42).

Another feature of reptile immunity that presents special challenges to diagnosis of infection by measuring seroconversionis the slow rate of specific antibody development. In the epidemiologicalsense (18), the sensitivity of a diagnostic test is the abilityof the test to identify individuals with the disease in the groupof diseased individuals. Specificity is the ability to identifyindividuals without disease in a healthy population. The positivepredictive value (PPV) is the ability to distinguish true infectionsin a population of individuals with positive test results, andthe negative predictive value (NPV) is the ability to distinguishtrue negative individuals from diseased individuals that havea negative test result. A reference standard that is independentof the assay being evaluated is required to estimate those parameters.In the dose-response and host range experiments, the referencestandard was experimental inoculation with 10⁶ CFU of M. alligatoris. Through 4 w.p.i., the sensitivity of theELISA was 0, the specificity was 100%, PPV was 0, and NPV wasonly 31% because specific antibody had not begun to appear. Evenat necropsy, the sensitivity was only 67%, the specificity was100%, PPV was 100%, and NPV was only 57% because half of the alligatorsand one-third of the caimans died before seroconversion couldoccur. Although those percentages are influenced by the numbersof experimental animals in the control and inoculated groups,they illustrate that the significance of the ELISA results, especiallynegative results, can change over time. An acutely lethal pathogensuch as M. alligatoris may escape serological detection at necropsyof crocodilians that die abruptly. Testing of paired samples,obtained at least 8 weeks apart, is necessary to minimize therisk of false-negative ELISAresults.

Surface-exposed epitopes on integral membrane proteins may be dominant immunogens during mycoplasmal infections (14). TheLAMP are anchored in the mycoplasmal membrane by covalent lipidmodification or hydrophobic transmembrane domains (2). In someexperiments, antibodies to LAMP antigens were highly mycoplasmaspecies specific and did not cross-react with LAMP from otherspecies (41). Therefore, LAMP immunogen-based diagnostics suchas ELISA promise high molecular specificity for some mycoplasmalspecies (15). Although M. alligatoris LAMP were among the prominentreactive antigens on Western immunoblots (Fig. 4), they did notgenerate a proportionate signal in the ELISA format for each speciesof crocodilian tested. The difference in antibody binding betweenformats may have been due to differences in quantity and typeof epitopes remaining exposed after denaturation and electrostaticbinding to nitrocellulose in the immunoblots versus coating ofthe native proteins onto hydrophilic polystyrene in theELISA.

The cross-reactivity with antigens of other mollicutes was in remarkable contrast to the lack of cross-reactivity observedin a similar whole-cell-lysate-based ELISA developed for tortoiseantibodies against M. agassizii (36). The difference may reflectdifferent immune system exposure to mycoplasmal antigens duringthe acute disease caused by highly invasive M. alligatoris, incontrast to the chronic disease caused by mucosa-tropic M. agassizii.The cross-reactivity may have been predominantly against internalmycoplasmal antigens conserved among mollicutes. This idea issupported by the complete lack of serological relationships betweenM. alligatoris and 71 other species of mollicutes assayed by reciprocalgrowth inhibition and colony surface immunofluorescence labelingtests (6). It was of concern that the alligators might possessexisting antibody against serum proteins or other mollicute culturemedium components potentially contaminating the mycoplasma lysateand LAMP preparations as a result of prior dietary exposure tothose antigens, which could confound the ELISA. However, cross-reactivitywith culture medium components was found to beinsignificant.

The results of the experimental inoculation studies described briefly above were remarkable because, except for bovine andcaprine pleuropneumonia, mycoplasmosis is rarely fatal in animals(29, 38). One other mycoplasmal disease of crocodilians hasbeen described. Polyarthritis was observed in young ranch-rearedNile crocodiles in Zimbabwe (26). At necropsy, M. crocodyli(19) was isolated from affected joints and lung tissue of thecrocodiles. The disease could be reproduced by experimental inoculationof crocodiles with M. crocodyli. Treatment with antibiotics seemedto resolve initial clinical signs, but relapses were common. Apreliminary study suggested that a vaccine might afford limitedprotection in young crocodiles (27). Although M. crocodyli andM. alligatoris are very closely related, as indicated by 98% 16SrRNA gene nucleotide sequence similarity (D. R. Brown, M. B. Brown,and J. G. Tully, Abstr. 97th Gen. Meet. Am. Soc. Microbiol., abstr.G-10, 1997), experimental intracoelomic or intrapleural inoculationof Nile crocodiles with 10⁹ CFU of M. crocodyli was not lethal (26, 27). However, a morerecent report associated M. crocodyli with a die-off of hundredsof ranched crocodiles (K. Mohan, C. M. Foggin, F. Dziva, and P.Muvavarirwa, Proc. 13th Int. Congr. Int. Org. Mycoplasmol., abstr.J-08, 2000). The susceptibility of alligators and caimans to infectionwith M. crocodyli remains unknown. An unidentified mycoplasmawas isolated from a gharial (Gavialis gangeticus) that died withpneumonia (25). Future study of the responses of the phylogeneticallyancient defense systems of crocodilians to M. alligatoris infectionmay allow unique comparative analyses of host-pathogen interactionsin mycoplasmaldisease.

	ACKNOWLEDGMENTS

This work was supported by U.S. Department of Agriculture NRICGP grant 9802614, Morris Animal Foundation grant 98ZO-44, andcontributions from the St. Augustine Alligator Farm and ZoologicalPark.

Technical assistance by Diane Duke (Interdisciplinary Center for Biotechnology Research) and Barbara Crenshaw (Departmentof Pathobiology) is gratefully acknowledged. Stuart Rosenberg(Silver Springs Wildlife Park, Ocala, Fla.), Yos Temsiripong (SrirachaCrocodile Farm, Sriracha, Thailand), and Sharon Deem (WildlifeConservation Society, Bronx, N.Y.) provided crocodilianplasma.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Pathobiology, College of Veterinary Medicine, University of Florida,Gainesville, FL 32611-0880. Phone: (352) 392-4700, ext. 3975.Fax: (352) 392-9704. E-mail: brownd{at}mail.vetmed.ufl.edu.

Present address: 8525 Richland Colony Rd., Knoxville, TN37923.

Present address: College of Veterinary Medicine and Animal Sciences, University of São Paulo, Botucatu SP 18618-000,Brazil.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Ambrosius, H. 1976. Immunoglobulins and antibody production in reptiles, p. 298-334. In J. J. Marchalonis (ed.), Comparative immunology. Blackwell Scientific Publications, Oxford, United Kingdom.

2. Bricker, T. M., M. J. Boyer, J. Keith, R. Watson-McKown, and K. S. Wise. 1988. Association of lipids with integral membrane surface proteins of Mycoplasma hyorhinis. Infect. Immun. 56:295-301[Abstract/Free Full Text].

3. Brown, D. R., B. C. Crenshaw, G. S. McLaughlin, I. M. Schumacher, C. E. McKenna, P. A. Klein, E. R. Jacobson, and M. B. Brown. 1995. Taxonomic analysis of the tortoise mycoplasmas Mycoplasma agassizii and Mycoplasma testudinis by 16S rRNA gene sequence comparisons. Int. J. Syst. Bacteriol. 45:348-350[CrossRef][Medline].

4. Brown, D. R., T. L. Clippinger, K. E. Helmick, I. M. Schumacher, R. A. Bennett, C. M. Johnson, K. A. Vliet, E. R. Jacobson, and M. B. Brown. 1996. Mycoplasma isolation during a fatal epizootic of captive alligators (Alligator mississippiensis) in Florida. Int. Org. Mycoplasmol. Lett. 4:42-43.

5. Brown, D. R., L. J. Richey, J. M. Johnson, E. R. Jacobson, K. A. Vliet, T. Gross, J. G. Tully, and M. B. Brown. 1998. Virulence and seroprevalence of a mycoplasmal pathogen of American alligators. Int. Org. Mycoplasmol. Lett. 5:103.

6. Brown, D. R., J. M. Johnson, L. A. Zacher, T. L. Clippinger, J. G. Tully, and M. B. Brown. Mycoplasma alligatoris sp. nov., a new species from American alligators. Int. J. Syst. Evol. Microbiol., in press.

7. Brown, M. B., G. S. McLaughlin, P. A. Klein, B. C. Crenshaw, I. M. Schumacher, D. R. Brown, and E. R. Jacobson. 1999. Upper respiratory tract disease in the gopher tortoise is caused by Mycoplasma agassizii. J. Clin. Microbiol. 37:2262-2269[Abstract/Free Full Text].

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13. Evans, A. S. 1976. Causation and disease: the Henle-Koch postulates revisited. Yale J. Biol. Med. 49:175-195[Medline].

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15. Gurevich, V. A., D. H. Ley, J. F. Markham, K. G. Whithear, and I. D. Walker. 1995. Identification of Mycoplasma synoviae immunogenic surface proteins and their potential use as antigens in the enzyme-linked immunosorbent assay. Avian Dis. 39:465-474[CrossRef][Medline].

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Antimicrob. Agents Chemother.	Clin. Microbiol. Rev.

Clin. Vaccine Immunol.	ALL ASM JOURNALS

1.	Ambrosius, H. 1976. Immunoglobulins and antibody production in reptiles, p. 298-334. In J. J. Marchalonis (ed.), Comparative immunology. Blackwell Scientific Publications, Oxford, United Kingdom.
2.	Bricker, T. M., M. J. Boyer, J. Keith, R. Watson-McKown, and K. S. Wise. 1988. Association of lipids with integral membrane surface proteins of Mycoplasma hyorhinis. Infect. Immun. 56:295-301[Abstract/Free Full Text].
3.	Brown, D. R., B. C. Crenshaw, G. S. McLaughlin, I. M. Schumacher, C. E. McKenna, P. A. Klein, E. R. Jacobson, and M. B. Brown. 1995. Taxonomic analysis of the tortoise mycoplasmas Mycoplasma agassizii and Mycoplasma testudinis by 16S rRNA gene sequence comparisons. Int. J. Syst. Bacteriol. 45:348-350[CrossRef][Medline].
4.	Brown, D. R., T. L. Clippinger, K. E. Helmick, I. M. Schumacher, R. A. Bennett, C. M. Johnson, K. A. Vliet, E. R. Jacobson, and M. B. Brown. 1996. Mycoplasma isolation during a fatal epizootic of captive alligators (Alligator mississippiensis) in Florida. Int. Org. Mycoplasmol. Lett. 4:42-43.
5.	Brown, D. R., L. J. Richey, J. M. Johnson, E. R. Jacobson, K. A. Vliet, T. Gross, J. G. Tully, and M. B. Brown. 1998. Virulence and seroprevalence of a mycoplasmal pathogen of American alligators. Int. Org. Mycoplasmol. Lett. 5:103.
6.	Brown, D. R., J. M. Johnson, L. A. Zacher, T. L. Clippinger, J. G. Tully, and M. B. Brown. Mycoplasma alligatoris sp. nov., a new species from American alligators. Int. J. Syst. Evol. Microbiol., in press.
7.	Brown, M. B., G. S. McLaughlin, P. A. Klein, B. C. Crenshaw, I. M. Schumacher, D. R. Brown, and E. R. Jacobson. 1999. Upper respiratory tract disease in the gopher tortoise is caused by Mycoplasma agassizii. J. Clin. Microbiol. 37:2262-2269[Abstract/Free Full Text].
8.	Clippinger, T. L., R. A. Bennett, C. M. Johnson, K. A. Vliet, S. L. Deem, J. Oros, E. R. Jacobson, I. M. Schumacher, D. R. Brown, and M. B. Brown. An epidemic of mycoplasmosis in captive alligators (Alligator mississippiensis) and transmission of the etiologic agent. J. Zoo Wildl. Med., in press.
9.	Cone, R. E., and J. J. Marchalonis. 1972. Cellular and humoral aspects of the influence of environmental temperature on the immune response of poikilothermic vertebrates. J. Immunol. 108:952-957[Abstract/Free Full Text].
10.	El Deeb, S. O., and A. H. M. Saad. 1990. Ontogenic maturation of the immune system in reptiles. Dev. Comp. Immunol. 14:151-159[CrossRef][Medline].
11.	El Ridi, R., N. Badir, and S. El Rouby. 1981. Effect of seasonal variations on the immune system of the snake, Psammophis schokari. J. Exp. Zool. 216:357-365[CrossRef].
12.	El Ridi, R., S. Zada, A. Afifi, S. El Deeb, S. El Rouby, M. Farag, and A.-H. Saad. 1988. Cyclic changes in the differentiation of lymphoid cells in reptiles. Cell Differ. 24:1-8[CrossRef][Medline].
13.	Evans, A. S. 1976. Causation and disease: the Henle-Koch postulates revisited. Yale J. Biol. Med. 49:175-195[Medline].
14.	Feng, S.-H., and S.-C. Lo. 1994. Induced mouse spleen B-cell proliferation and secretion of immunoglobulin by lipid-associated membrane proteins of Mycoplasma fermentans incognitus and Mycoplasma penetrans. Infect. Immun. 62:3916-3921[Abstract/Free Full Text].
15.	Gurevich, V. A., D. H. Ley, J. F. Markham, K. G. Whithear, and I. D. Walker. 1995. Identification of Mycoplasma synoviae immunogenic surface proteins and their potential use as antigens in the enzyme-linked immunosorbent assay. Avian Dis. 39:465-474[CrossRef][Medline].
16.	Horowitz, S. A., and G. H. Cassell. 1978. Detection of antibodies to Mycoplasma pulmonis by an enzyme-linked immunosorbent assay. Infect. Immun. 22:161-170[Abstract/Free Full Text].
17.	Jeffcoate, S. L. 1982. Use of Youden plot for internal quality control in the immunoassay laboratory. Ann. Clin. Biochem. 19:435-437[Medline].
18.	Kenny, G. E. 1992. Serodiagnosis, p. 505-512. In J. Maniloff, R. N. McElhaney, L. R. Finch, and J. B. Baseman (ed.), Mycoplasmas: molecular biology and pathogenesis. American Society for Microbiology, Washington, D.C.
19.	Kirchhoff, H., K. Mohan, R. Schmidt, M. Runge, D. R. Brown, M. B. Brown, C. M. Foggin, P. Muvavarirwa, H. Lehmann, and J. Flossdorf. 1997. Mycoplasma crocodyli sp. nov., a new species from crocodiles. Int. J. Syst. Bacteriol. 47:742-746[CrossRef][Medline].
20.	Leceta, J., and A. Zapata. 1986. Seasonal variations in the immune response of the tortoise Mauremys caspica. Immunology 57:483-487[Medline].
21.	Lerch, E. G., S. E. Huggins, and A. H. Bartel. 1967. Comparative immunology: active immunization of young alligators with hemocyanin. Proc. Soc. Exp. Biol. Med. 124:448-451[Medline].
22.	Levisohn, S., R. Rosengarten, and D. Yogev. 1995. In vivo variation of Mycoplasma gallisepticum antigen expression in experimentally infected chickens. Vet. Microbiol. 45:219-231[CrossRef][Medline].
23.	Maniloff, J. 1992. Phylogeny of mycoplasmas, p. 549-559. In J. Maniloff, R. N. McElhaney, L. R. Finch, and J. B. Baseman (ed.), Mycoplasmas: molecular biology and pathogenesis. American Society for Microbiology, Washington, D.C.
24.	Maung, R. T. 1963. Immunity in the tortoise Testudo ibera. J. Pathol. Bacteriol. 85:51-66[CrossRef][Medline].
25.	Misra, P. R., S. K. Patra, H. K. Mohapatra, K. C. Patra, and S. Mohapatra. 1996. Aetiopathological findings from young gharial mortality cases. Indian Vet. J. 73:888-889.
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